Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP

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Bacteriophage Recombineering of Electroporated DNA (BRED) has been described for construction of gene deletion and point mutations in mycobacteriophages. Using BRED, we inserted a Phsp60-egfp cassette (1143 bp) into the mycobacteriophage D29 genome to construct a new reporter phage, which was used f...

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Autores principales: da Silva, J.L., Piuri, M., Broussard, G., J. Marinelli, L., Bastos, G.M., Hirata, R.D.C., Hatfull, G.F., Hirata, M.H.
Formato: Artículo publishedVersion
Publicado: 2013
Materias:
Bacteriophage
Green fluorescent protein
Mycobacterium
Recombineering
DNA
enhanced green fluorescent protein
genomic DNA
analytic method
article
bacteriophage
Bacteriophage Recombineering of Electroporated DNA technology
cytolysis
DNA sequence
gene cassette
gene deletion
gene mutation
nonhuman
point mutation
priority journal
protein expression
Electroporation
Genes, Reporter
Green Fluorescent Proteins
Lysogeny
Mycobacteriophages
Mycobacterium smegmatis
Promoter Regions, Genetic
Sequence Deletion
Acceso en línea:http://hdl.handle.net/20.500.12110/paper_03781097_v344_n2_p166_daSilva
http://repositoriouba.sisbi.uba.ar/gsdl/cgi-bin/library.cgi?a=d&c=artiaex&d=paper_03781097_v344_n2_p166_daSilva_oai
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Repositorio Digital de la Universidad de Buenos Aires (UBA) de Universidad de Buenos Aires
id I28-R145-paper_03781097_v344_n2_p166_daSilva_oai
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spelling I28-R145-paper_03781097_v344_n2_p166_daSilva_oai2020-10-19 da Silva, J.L. Piuri, M. Broussard, G. J. Marinelli, L. Bastos, G.M. Hirata, R.D.C. Hatfull, G.F. Hirata, M.H. 2013 Bacteriophage Recombineering of Electroporated DNA (BRED) has been described for construction of gene deletion and point mutations in mycobacteriophages. Using BRED, we inserted a Phsp60-egfp cassette (1143 bp) into the mycobacteriophage D29 genome to construct a new reporter phage, which was used for detection of mycobacterial cells. The cassette was successfully inserted and recombinant mycobacteriophage purified. DNA sequencing of the cassette did not show any mutations even after several phage generations. Mycobacterium smegmatis mc2155 cells were infected with D29::Phsp60-egfp (MOI of 10) and evaluated for EGFP expression by microscopy. Fluorescence was observed at around 2 h after infection, but dissipated in later times because of cell lysis. We attempted to construct a lysis-defective mutant by deleting the lysA gene, although we were unable to purify the mutant to homogeneity even with complementation. These observations demonstrate the ability of BRED to insert c. 1 kbp-sized DNA segments into mycobacteriophage genomes as a strategy for constructing new diagnostic reporter phages. © 2013 Federation of European Microbiological Societies. Published by John Wiley & Sons Ltd. Fil:Piuri, M. Universidad de Buenos Aires. Facultad de Ciencias Exactas y Naturales; Argentina. application/pdf http://hdl.handle.net/20.500.12110/paper_03781097_v344_n2_p166_daSilva info:eu-repo/semantics/openAccess http://creativecommons.org/licenses/by/2.5/ar FEMS Microbiol. Lett. 2013;344(2):166-172 Bacteriophage Green fluorescent protein Mycobacterium Recombineering DNA enhanced green fluorescent protein genomic DNA analytic method article bacteriophage Bacteriophage Recombineering of Electroporated DNA technology cytolysis DNA sequence gene cassette gene deletion gene mutation nonhuman point mutation priority journal protein expression Electroporation Genes, Reporter Green Fluorescent Proteins Lysogeny Mycobacteriophages Mycobacterium smegmatis Promoter Regions, Genetic Sequence Deletion Mycobacterium Mycobacterium smegmatis Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP info:eu-repo/semantics/article info:ar-repo/semantics/artículo info:eu-repo/semantics/publishedVersion http://repositoriouba.sisbi.uba.ar/gsdl/cgi-bin/library.cgi?a=d&c=artiaex&d=paper_03781097_v344_n2_p166_daSilva_oai
institution Universidad de Buenos Aires
institution_str I-28
repository_str R-145
collection Repositorio Digital de la Universidad de Buenos Aires (UBA)
topic Bacteriophage
Green fluorescent protein
Mycobacterium
Recombineering
DNA
enhanced green fluorescent protein
genomic DNA
analytic method
article
bacteriophage
Bacteriophage Recombineering of Electroporated DNA technology
cytolysis
DNA sequence
gene cassette
gene deletion
gene mutation
nonhuman
point mutation
priority journal
protein expression
Electroporation
Genes, Reporter
Green Fluorescent Proteins
Lysogeny
Mycobacteriophages
Mycobacterium smegmatis
Promoter Regions, Genetic
Sequence Deletion
Mycobacterium
Mycobacterium smegmatis
spellingShingle Bacteriophage
Green fluorescent protein
Mycobacterium
Recombineering
DNA
enhanced green fluorescent protein
genomic DNA
analytic method
article
bacteriophage
Bacteriophage Recombineering of Electroporated DNA technology
cytolysis
DNA sequence
gene cassette
gene deletion
gene mutation
nonhuman
point mutation
priority journal
protein expression
Electroporation
Genes, Reporter
Green Fluorescent Proteins
Lysogeny
Mycobacteriophages
Mycobacterium smegmatis
Promoter Regions, Genetic
Sequence Deletion
Mycobacterium
Mycobacterium smegmatis
da Silva, J.L.
Piuri, M.
Broussard, G.
J. Marinelli, L.
Bastos, G.M.
Hirata, R.D.C.
Hatfull, G.F.
Hirata, M.H.
Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
topic_facet Bacteriophage
Green fluorescent protein
Mycobacterium
Recombineering
DNA
enhanced green fluorescent protein
genomic DNA
analytic method
article
bacteriophage
Bacteriophage Recombineering of Electroporated DNA technology
cytolysis
DNA sequence
gene cassette
gene deletion
gene mutation
nonhuman
point mutation
priority journal
protein expression
Electroporation
Genes, Reporter
Green Fluorescent Proteins
Lysogeny
Mycobacteriophages
Mycobacterium smegmatis
Promoter Regions, Genetic
Sequence Deletion
Mycobacterium
Mycobacterium smegmatis
description Bacteriophage Recombineering of Electroporated DNA (BRED) has been described for construction of gene deletion and point mutations in mycobacteriophages. Using BRED, we inserted a Phsp60-egfp cassette (1143 bp) into the mycobacteriophage D29 genome to construct a new reporter phage, which was used for detection of mycobacterial cells. The cassette was successfully inserted and recombinant mycobacteriophage purified. DNA sequencing of the cassette did not show any mutations even after several phage generations. Mycobacterium smegmatis mc2155 cells were infected with D29::Phsp60-egfp (MOI of 10) and evaluated for EGFP expression by microscopy. Fluorescence was observed at around 2 h after infection, but dissipated in later times because of cell lysis. We attempted to construct a lysis-defective mutant by deleting the lysA gene, although we were unable to purify the mutant to homogeneity even with complementation. These observations demonstrate the ability of BRED to insert c. 1 kbp-sized DNA segments into mycobacteriophage genomes as a strategy for constructing new diagnostic reporter phages. © 2013 Federation of European Microbiological Societies. Published by John Wiley & Sons Ltd.
format Artículo
Artículo
publishedVersion
author da Silva, J.L.
Piuri, M.
Broussard, G.
J. Marinelli, L.
Bastos, G.M.
Hirata, R.D.C.
Hatfull, G.F.
Hirata, M.H.
author_facet da Silva, J.L.
Piuri, M.
Broussard, G.
J. Marinelli, L.
Bastos, G.M.
Hirata, R.D.C.
Hatfull, G.F.
Hirata, M.H.
author_sort da Silva, J.L.
title Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
title_short Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
title_full Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
title_fullStr Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
title_full_unstemmed Application of BRED technology to construct recombinant D29 reporter phage expressing EGFP
title_sort application of bred technology to construct recombinant d29 reporter phage expressing egfp
publishDate 2013
url http://hdl.handle.net/20.500.12110/paper_03781097_v344_n2_p166_daSilva
http://repositoriouba.sisbi.uba.ar/gsdl/cgi-bin/library.cgi?a=d&c=artiaex&d=paper_03781097_v344_n2_p166_daSilva_oai
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